Specific nutritional or therapeutic agent including a mixture of grape and blueberry

ABSTRACT

The invention concerns a nutritional or therapeutic agent comprising a molecule mix obtained from  Vitis vinifera  and  Vaccinium angustifolium , comprising:
         at least 1% of catechins and epicatechins, the percentage being given by weight in relation to the total weight of the mix, preferably at least 5%,   at least 5 ppm (parts per million in the mix) of ferulic acid, preferably at least 10 ppm.       

     The invention also relates to the use of this agent due to its effects on cognitive functions in particular.

CROSS-REFERENCE TO RELATED APPLICATIONS

This application is a continuation application of U.S. patent application Ser. No. 15/771,328 filed Apr. 26, 2018 which is a U.S. national stage application of PCT/EP2016/075905 filed Oct. 27, 2016 which claims a benefit of priority from French patent application FR 1560263 filed Oct. 27, 2015, the entire disclosures of which are herein incorporated by reference.

TECHNICAL FIELD

This invention relates to a mixture of specific polyphenols having a synergistic action particularly on the cognitive functions and executive functions in humans and animals.

The invention also covers the use of this mixture to improve cognitive functions and executive functions, delay cognitive decline and prevent and combat the pathologies associated with cognitive decline in humans and animals.

BACKGROUND

It is known that old age is associated with cognitive disorders and neurodegenerative deficits such as Alzheimer's disease and Parkinson's disease. As the elderly population increases, there is a prevalence of these age-related disorders. It is therefore important to develop solutions to prevent or minimize age-related cognitive decline and delay the appearance of associated pathologies.

To this end, a prevention based on nutrition has been suggested over recent years to avoid or delay the development towards dementia and thus maintain a stable cognitive state and wellbeing in the elderly. Research dedicated to understanding the relationship between nutrition and “healthy aging” has thus intensified and among the foods studied, fruits and vegetables rich in polyphenols have been identified as capable of delaying age-related physiological and functional deficits and protecting humans or animals against associated degenerative diseases (as described for example in: Joseph J A, Shukitt-Hale B, Casadesus G “Reversing the deleterious effects of aging on neuronal communication and behavior: beneficial properties of fruit polyphenolic compounds” in the American Journal of Clinical Nutrition 2005; 81 (Suppl 1): 313S-6S.). In fact, polyphenols, particularly flavonoids, are known for their ability to improve the learning process and memory and are now widely studied for their potential in the prevention of age-related cognitive decline in both animals and humans. Although the mechanisms of action of flavonoids are not clearly identified, they are known to be capable of modifying the cellular and molecular processes involved in learning and memory.

Included among the fruits containing polyphenols, studied for their effect on age-related cognitive decline, are berries in particular, and specifically blueberries, strawberries and grapes. Among the different polyphenols present in berries, those that have been specifically studied for their effect on brain functions are resveratrol and flavonoids, particularly flavanols and anthocyanins.

Blueberries are known to contain a large quantity of polyphenols and have a greater antioxidant capacity than other fruits and vegetables. Numerous studies suggest that the consumption of blueberries delays age-related functional and physiological deficits. For example, daily consumption of blueberry juice for 12 weeks improves the performance of episodic memory in the elderly (Krikorian R, Shidler M D, Nash T A, Kalt W, Vinqvist-Tymchuk M R, Shukitt-Hale B, et al. «Blueberry supplementation improves memory in older adults”. Journal of Agricultural and Food Chemistry. 2010; 58(7):3996-4000).

Strawberries have a strong antioxidant and anti-inflammatory power capable of preventing age-related neurochemical and behavioral changes.

As for grapes, they are particularly rich in flavonoids (catechins, epicatechins, proanthocyanidin oligomers, procyanidin polymers and anthocyanins) known for their powerful antioxidant capacities. The nutritional properties of grapes like the source of polyphenols in wine also form the subject of numerous studies. Similar to the results obtained with blueberry juice, the consumption of grape juice for 12 weeks leads to an improvement in memory performance in the elderly (Krikorian R, Nash T A, Shidler M D, Shukitt-Hale B, Joseph J A. «Concord grape juice supplementation improves memory function in older adults with mild cognitive impairment.” The British Journal of Nutrition. 2010; 103(5):730-4). Moreover, specific grape extracts (grape seed extracts, for example) are now used as a nutritional supplement due to their high concentration of polyphenols, particularly flavanols, anthocyanins and resveratrol. These extracts are suitable for nutritional supplementation because they contain a higher polyphenol concentration than fruits or juices, which facilitates the identification of their effects and the study of underlying neurobiological mechanisms. The use of berries, juices or extracts of berries to delay age-related cognitive decline and improve brain functions is therefore known. However, when humans or animals consume existing berries, juices or extracts of berries, the bioavailability of the polyphenols contained in these products is unsatisfactory and the effect on cognitive and functional functions is insufficient.

Thus, the aim of the invention is to overcome these drawbacks by proposing a product that contains polyphenols having an improved bioavailability and greater efficiency for combatting cognitive decline.

SUMMARY

To this end, the invention concerns a nutritional or therapeutic agent comprising a molecule mix obtained from Vitis vinifera and Vaccinium angustifolium, comprising:

-   -   at least 1% of catechin and/or epicatechin, the percentage being         given by weight in relation to the total weight of the mix,         preferably at least 5%,     -   at least 5 ppm (parts per million in the mix) of ferulic acid,         preferably at least 10 ppm.

The agent according to the invention contains flavanols, in particular catechins and/or epicatechins, known for their effect on cognitive performance, as specifically described in Endeiro C, Vauzour D, Rattray M, Waffo-Teguo P, Merillon J M, Butler L T, et al. “Dietary levels of pure flavonoids improve spatial memory performance and increase hippocampal brain- derived neurotrophic factor” PloS one. 2013; 8(5):e63535, as well as Van Praag H, Lucero M J, Yeo G W, Stecker K, Heivand N, Zhao C, et al. “Plant-derived flavanol (−)epicatechin enhances angiogenesis and retention of spatial memory in mice”. The Journal of Neuroscience: the official journal of the Society for Neuroscience. 2007; 27(22):5869-78.

Similarly, ferulic acid is known for its effects on the nervous system, particularly to protect neuronal cells from cell death caused by cerebral ischemia as described specifically in Cheng C Y S, S. Y.; Tang, N. Y.; Ho, T. Y.; Chiang, S. Y.; Hsieh, C. L. “Ferulic acid provides neuroprotection against oxidative stress-related apoptosis after cerebral ischemia/reperfusion injury by inhibiting ICAM-1 mRNA expression in rats”. Brain Res. 2008; 1209:136-50. Moreover, its antioxidant activity has been tested in Alzheimer's disease (Sgarbossa A, Giacomazza D, Di Carlo M. “Ferulic Acid: A Hope for Alzheimer's Disease Therapy from Plants. Nutrients”. 2015; 7(7):5764-82) and its long-term administration seems to protect against memory and learning deficits (Yan J J C, J. Y.; Kim, H. S.; Kim, K. L.; Jung, J. S.; Huh, S. O.; Suh, H. W.; Kim, Y. H.; Song, D. K. “Protection against 6-amyloid peptide toxicity in vivo with long-term administration of ferulic acid”. Br J Pharmacol. 2001; 133:89-96).

This effect is further increased when the agent also comprises:

-   -   at least 200 ppm of resveratrol, and/or     -   at least 50 ppm of quercetin and/or quercetin glycosides, and/or     -   at least 500 ppm of anthocyanidins.

These molecules are also known for their effect on cognitive functions.

Resveratrol also has numerous beneficial activities for humans or animals, including an improvement in working memory, learning and spatial memory and spontaneous motor activity (Abraham J, Johnson R W. «Consuming a diet supplemented with resveratrol reduced infection-related neuroinflammation and deficits in working memory in aged mice”. Rejuvenation research. 2009; 12(6):445-53; Dal-Pan A, Pifferi F, Marchal J, Picq J L, Aujard F. “Cognitive performances are selectively enhanced during chronic caloric restriction or resveratrol supplementation in a primate”. PloS one. 2011; 6(1):e16581. Resveratrol is particularly known for possibly being present in grapes, but is not present in all grape extracts. In fact, resveratrol is a phytoalexin that develops basically on the grape skin in a very variable manner and its presence in extracts, as with other molecules, is also dependent on the extraction method used.

Quercetin also has a significant neuroprotective action (Dajas F, Andres A C, Florencia A, Carolina E, Felicia R M. “Neuroprotective actions of flavones and flavonols: mechanisms and relationship to flavonoid structural features. Central nervous system agents in medicinal chemistry.” 2013; 13(1):30-5.) and it is also known that the consumption of foods rich in anthocyanidins prevents memory deficiencies and improves cognitive performance (Barros D, Amaral O B, Izquierdo I, Geracitano L, do Carmo Bassols Raseira M, Henriques A T, et al. “Behavioral and genoprotective effects of Vaccinium berries intake in mice”. Pharmacology, Biochemistry, and Behavior. 2006; 84(2):229-34; Cho J, Kang J S, Long P H, Jing J, Back Y, Chung K S. “Antioxidant and memory enhancing effects of purple sweet potato anthocyanin and cordyceps mushroom extract. Archives of Pharmacal Research”. 2003; 26(10):821-5; Ramirez M R, Izquierdo I, do Carmo Bassols Raseira M, Zuanazzi J A, Barros D, Henriques A T. “Effect of lyophilised Vaccinium berries on memory, anxiety and locomotion in adult rats. Pharmacological Research: the official journal of the Italian Pharmacological Society”. 2005; 52(6):457-62.).

Surprisingly, the combination and specific quantity of polyphenols present in the agent has a synergistic effect and increases the bioavailability of the polyphenols when they are administered to humans or animals in comparison to the bioavailability of these same polyphenols when they are administered in isolation or via existing berry extracts or when consuming grapes or blueberries or at different concentrations in existing products. The molecules of the mixture and consequently the agent according to the invention have in particular an antioxidant synergistic effect and/or an effect on the improvement of cognitive and/or executive functions in humans or animals.

The agent according to the invention is therefore particularly useful notably as a drug for humans or animals, and specifically to prevent and/or combat pathologies associated with cognitive decline.

Similarly, the invention also concerns the use of such an agent for non-therapeutic nutritional applications in healthy humans or animals, particularly to improve cognitive and/or executive functions.

BRIEF DESCRIPTION OF THE DRAWINGS

The invention is now described in detail with reference to the accompanying figures, in which:

FIG. 1 shows the differences in bioavailability of polyphenols in mouse plasma, between an acute administration and a chronic administration of an extract of Vitis vinifera, an extract of Vaccinium angustifolium or of an agent according to the invention;

FIG. 2 shows the ascending hierarchical classification (AHC) of the phenolic metabolites found in mouse plasma before and after treatment by chronic ingestion of an extract of Vitis vinifera, an extract of Vaccinium angustifolium or of an agent according to the invention;

FIG. 3 shows the ascending hierarchical classification (AHC) of the phenolic metabolites found in mouse excrement before and after treatment by chronic ingestion of an extract of Vitis vinifera, of an extract of Vaccinium angustifolium or of an agent according to the invention;

FIG. 4A shows the effects of ferulic acid only on the protection of neuronal cells after an acute treatment;

FIG. 4B shows the effects of catechin only on the protection of neuronal cells after an acute treatment;

FIG. 4C shows the effects of epicatechin only on the protection of neuronal cells after an acute treatment;

FIG. 4D shows the effects of the agent according to the invention on the protection of neuronal cells after an acute treatment;

FIG. 5A shows the effects of ferulic acid only, catechin only and epicatechin only on the protection of neuronal cells after three cumulative treatments (cell survival);

FIGS. 5B, 5C, 5D and 5E show the effects of the agent according to the invention on the protection of neuronal cells after three cumulative treatments at different concentrations (cell survival);

FIG. 5F shows the effects of the agent according to the invention on the protection of neuronal cells after three cumulative treatments (production of ROS);

FIG. 6 represents the total antioxidant status (TAS) of adult dogs having been treated with the agent according to the invention, an extract of Vitis vinifera, an extract of Vaccinium angustifolium, and a control;

FIG. 7 shows the effect on the cognitive functions of dogs of an agent according to the invention at different doses, in comparison to a placebo.

DETAILED DESCRIPTION

The subject matter of the invention therefore concerns a nutritional or therapeutic agent comprising at least one molecule mix obtained from Vitus vinifera and Vaccinium angustifolium, said mix comprising:

-   -   at least 1% of catechin and/or epicatechin, the percentage being         given by weight in relation to the total weight of the mix,         preferably at least 5%, even more preferably between 5% and 50%,         specifically between 7% and 35%,     -   at least 5 ppm (parts per million in the mix) of ferulic acid,         preferably at least 10 ppm, even more preferably between 5 ppm         and 300 ppm, specifically between 10 ppm and 100 ppm.

Preferably, in addition to the at least 1% of catechin and/or epicatechin, and at least 5 ppm of ferulic acid, the molecule mix according to the invention also comprises:

-   -   at least 200 ppm of resveratrol, preferably at least 300 ppm,         even more preferably at least 400 ppm, even more preferably         between 300 ppm and 6000 ppm, specifically between 400 and 6000         ppm, and/or     -   at least 50 ppm of quercetin and/or quercetin glycosides,         preferably at least 70 ppm of quercetin and/or glycoside,         specifically between 50 ppm and 10000 ppm, and/or     -   at least 500 ppm of anthocyanidins, preferably at least 600 ppm,         even more preferably at least 700 ppm, even more preferably         between 600 ppm and 5000 ppm.

Preferably, malvidin 3-glucoside is the preponderant anthocyanidin. It is preferably present at a concentration of at least 300 ppm in the mix.

“Nutritional agent” in the sense of the invention means a food ingredient with a nutritional purpose used alone or associated with other food ingredients or additives in food formulas including food supplements intended for humans or animals.

“Therapeutic agent” in the sense of the invention means an active ingredient used for therapeutic purposes alone or associated with other active substances or not in drug formulas including phytotherapy, intended for humans or animals.

“Anthocyanidin” in the sense of the invention means all anthocyanins or anthocyanosides, in aglycone or glycosylated form (i.e. bearing sugars). Thus, in the present application and in the sense of the present invention, the terms “anthocyanidin”, “anthocyanins” and “anthocyanosides” are equivalent.

“At least X % of catechins and/or epicatechins” means either at least X % of catechins if there are no epicatechins in the mix, or at least X % of epicatechins if there are no catechins in the mix, or at least X % of the mix of catechins and epicatechins if both catechins and epicatechins are present in the mix at the same time. Preferably, this means at least X % of the mix of catechins and epicatechins.

“Ppm” means parts per million (mg/kg) in the mix. Unless stated otherwise, ppm refers to a weight in relation to the total weight of the mix.

According to a first embodiment, the molecule mix is a mixture formed by an extract of Vitis vinifera and an extract of Vaccinium angustifolium.

According to a second embodiment, the molecule mix is a mixture formed by an extract obtained from a mixture of Vitis vinifera and Vaccinium angustifolium.

According to a third embodiment, the molecule mix is a mixture formed by:

-   -   an extract of Vitis vinifera and/or an extract of Vaccinium         angustifolium, and     -   an extract obtained from a mixture of Vitis vinifera and         Vaccinium angustifolium.

“Extract of Vitis vinifera” in the sense of the invention means at least one molecule preferably a collection of molecules, obtained from Vitis vinifera. The raw material can be the leaves and/or fruits and/or seeds and/or wood, preferably the raw material is the above-ground part of the plant, i.e. the leaves, fruits, pellicle (i.e. the skin), seeds and wood, even more preferably the skin (pellicle) and seeds. The association of the skin, which can be rich in resveratrol, and the seeds, which can be rich in flavanol monomers, in procyanidin oligomers and in proanthocyanidins, can be particularly advantageous for the invention.

Preferably, the extract of Vitis vinifera is an extract having a flavanol polymer content of less than 0.5% by weight of the total weight of the polyphenols of the extract, even more preferably a content of less than 0.1%. “Flavanol polymer” means a flavanol having a degree of polymerisation of more than 10. According to the invention, the flavanol polymers have very little bioavailability, unlike flavanol monomers that are very quickly absorbed into the small intestine then metabolized into methylated, sulfated and glucuronidated derivatives.

This low presence of polymers is a quality criterion of grape extracts used in particular due to their efficacy and bioavailability.

“Extract of Vaccinium angustifolium” in the sense of the invention means at least one molecule, preferably a combination of molecules, obtained from Vaccinium angustifolium. The raw material can be the leaves and/or fruits, preferably the raw material is the combination of the leaves and fruits of the plant.

Extract obtained from a mixture of Vitis vinifera and Vaccinium angustifolium means a combination of molecules obtained from a mixture of Vitis vinifera and Vaccinium angustifolium. The raw material of Vitis vinifera can be the leaves and/or the fruits and/or the seeds and/or the wood, preferably the raw material of Vitis vinifera is the above-ground part of the plant, i.e. the combination of leaves, fruit, skin (pellicle), seeds and wood, more preferably the skin (pellicle) and seeds. The raw material of Vaccinium angustifolium can be the leaves and/or fruits, preferably the raw material of Vaccinium angustifolium is the combination of the leaves and fruits of the plant.

The extract according to the invention can be obtained by any method allowing a mix to be obtained that comprises:

-   -   at least 1% of catechin and/or epicatechin by weight in relation         to the total weight of the mix, preferably at least 5%, even         more preferably between 5% and 50%, specifically between 7% and         35%,     -   at least 5 ppm of ferulic acid, preferably at least 10 ppm, even         more preferably between 5 ppm and 300 ppm, specifically between         10 ppm and 100 ppm,     -   optionally, at least 200 ppm of resveratrol, preferably at least         300 ppm, even more preferably at least 400 ppm, even more         preferably between 300 ppm and 6000 ppm, specifically between         400 and 6000 ppm,     -   optionally, at least 50 ppm, of quercetin and/or quercetin         glycosides, preferably at least 70 ppm, of quercetin and/or         glycoside, specifically between 50 ppm and 10000 ppm,     -   optionally, at least 500 ppm of anthocyanidins, preferably at         least 600 ppm, even more preferably at least 700 ppm, even more         preferably between 600 ppm and 5000 ppm.

Preferably malvidin 3-glucoside is the preponderant anthocyanidin with a concentration of at least 300 ppm. Preferably, the anthocyanidins comprise at least 20%, more preferably at least 25% of malvidin 3-glucoside (percentage by weight).

A particularly appropriate method is a method comprising the following steps:

-   -   obtaining an extract of Vitis vinifera:         -   water and/or ethanol extraction of Vitis vinifera,             preferably from the combination of leaves, fruits, pellicle,             seeds and wood of Vitis vinifera. The quantity of solvent             (30% v/v to 96% v/v) used is between 2 and 10 times the mass             of material used. The duration of the extraction can be             between 30 minutes and 24 hours and the extraction             temperature between 20° C. and 80° C. The raw materials used             can be in dry, fresh or whole frozen or ground form;         -   separation of the solution of water and/or ethanol from the             solid matter, for example by centrifugal decantation or by             pressing and filtration;         -   evaporation of the ethanol under vacuum evaporation at a             temperature preferably below 60° C. and at a pressure below             100 mbars;         -   membrane separation of the extract previously de-solvented             so as preferably to select the proanthocyanidic monomers and             oligomers (having a degree of polymerization of between 2             and 10 inclusive) and eliminate the flavanol polymers             (>decamers), in order to obtain an extract characterized by             a flavanol polymer content of less than 0.5% and more             preferably less than 0.1% by weight in relation to the total             weight of the polyphenols of the extract. This step can be             performed with the aid of a filtration membrane having a             cut-off threshold of less than 15000 daltons and more             preferably less than 3000 daltons;     -   obtaining an extract of Vaccinium angustifolium:         -   water and/or ethanol extraction of Vaccinium angustifolium,             preferably from the leaves and fruits of Vaccinium             angustifolium. The quantity of solvent (30% v/v to 96% v/v)             used is between 2 and 10 times the mass of material used.             The duration of the extraction can be between 30 minutes and             24 hours and the extraction temperature between 20° C. and             80° C. The raw materials used can be in dry, fresh or frozen             form;         -   separation of the solution of water and/or ethanol from the             solid matter by centrifugal decantation or by pressing and             filtration;         -   evaporation of the ethanol under vacuum evaporation at a             temperature preferably below 60° C. and at a pressure below             100 mbars;     -   drying the extracts by spray drying, in a vacuum oven or by         freeze drying with or without a support such as a maltodextrin;     -   mixing the extract of Vitis vinifera and Vaccinium angustifolium         before or after the drying step.

According to a variation, the method consists in implementing the following steps:

-   -   mixing Vitis vinifera and Vaccinium angustifolium, water and/or         ethanol extraction of Vaccinium angustifolium, preferably from         the combination of the leaves and fruits of Vaccinium         angustifolium. The quantity of solvent (30% v/v to 96% v/v) used         is between 2 and 10 times the mass of material used. The         duration of the extraction can be between 30 minutes and 24         hours and the extraction temperature between 20° C. and 80° C.         The raw materials used can be in dry, fresh or frozen form;     -   separation of the solution of water and/or ethanol from the         solid pomace by centrifugal decantation or by pressing and         filtration;     -   evaporation of the ethanol under vacuum evaporation at a         temperature preferably below 60° C. and at a pressure below 100         mbars;     -   drying the extract by spraying or sublimation with or without a         support such as maltodextrin.

Whatever the variation of the method, before the drying step, the method can comprise the following steps:

-   -   loading onto a resin of solutions of mixed or unmixed extracts,     -   rinsing the resin with water,     -   applying an eluent solution of water/ethanol onto the resin,     -   recovering the purified eluate,     -   evaporating the ethanol from said eluate,     -   concentrating said eluate,     -   drying said purified aqueous extract.

The nutritional or therapeutic agent according to the invention can consist exclusively of a mixture of molecules, i.e. extracts, or comprise other constituents. Preferably, in addition to the mixture of molecules, the nutritional or therapeutic agent according to the invention contains other constituents, in particular excipients or coating agents, such as maltodextrin, microcrystalline cellulose, cyclodextrins, starch and soluble or insoluble fibers.

The agent can be in any form suitable for a nutritional or therapeutic application, preferably in powder form.

The agent according to the invention can be incorporated in a composition, in particular in a nutritional or therapeutic (drug) composition if in a form chosen from tablets, capsules, gel capsules, powders, solutions, microcapsules, suspensions, emulsions, food supplements, drinks and food for humans or animals.

It may be a non-therapeutic nutritional composition intended for humans such as, for example, food supplements, bars, dairy products, powders to be swallowed or rehydrated, gels, jams, sweets, carbonated and non-carbonated beverages, dry beverages to be rehydrated and compotes.

It may also be a drug intended for humans such as, for example, tablets or capsules.

It may also be a nutritional or therapeutic composition intended for animals. An “animal” means any animal capable of receiving a nutritional or therapeutic agent according to the invention, for example but in a non-limiting manner a pet, a fowl, a pig, a ruminant, a goat or even a mouse. Preferably, the animal is a pet, such as a cat or dog. More preferably, the animal is a dog.

It may also be a non-therapeutic nutritional composition intended for an animal such as, for example, dry foods, such as kibbles (extruded, co-extruded or freeze dried), treats, snacks, wet or semi-wet foods such as pieces in sauce, chunks in jelly, beverages, or even food supplements. Preferably, the agent is incorporated in dry foods such as kibbles.

Lastly, it can be a drug intended for animals, or a veterinary product, such as, for example, tablets, capsules, sprays and liquids administered dropwise.

Advantageously, the agent intended for animals can be incorporated into a composition, in particular into a nutritional or therapeutic composition, as an inclusion, namely by adding it to the mass of the composition for example by impregnation or mixing, or as a coating, namely by applying it to the surface of the composition, by spraying or by dusting, for example by mixing it beforehand with one or more ingredients such as at least one palatability enhancer. The nutritional or therapeutic agent can be used in particular to act on the cognitive and executive functions in a healthy individual or animal but also in sick subjects.

Cognitive decline is characterized by an age-related reduction in the cognitive and executive functions, particularly concentration, work, long-term memory, ability to reason, judge, solve problems and speed of processing information. These deficiencies can lead to a reduction in self-esteem and quality of life. Age-related cognitive decline is the term used to described the non-pathological form of the deterioration of memory and cognitive functions resulting from the aging process within normal limits, taking into account a person's age. This is a complex process, with the first signs emerging in humans between 35 and 65 years, with no specific neurodegenerative lesions. Gradual cognitive decline can be manifested by the appearance of minor cognitive problems that affect 15 to 20% of the population aged 65 or over, but that represent an unstable condition. However, certain pathological forms can arise in addition to this “normal” cognitive decline. Among these pathologies, Alzheimer's disease is the most common cause of dementia, affecting over 24 million people worldwide. It is irreversible within our current state of knowledge, the only treatments available being purely symptomatic. In animals, these pathologies can manifest themselves in a very similar manner.

In dogs, for example, cognitive dysfunction syndrome (or CDS) is a widespread pathology characterized by spatio-temporal disorientation, a loss of elementary learning that often leads to uncleanliness, a change in sleep/wake cycles and a change in social interactions.

The agent according to the invention is capable of improving the cognitive and executive functions in humans or animals. The association of two raw materials and the specificity of the extracts according to the invention comprising polyphenols combined in specific quantities, produces a synergistic effect in comparison to polyphenols taken alone or to existing extracts containing polyphenols in different proportions and quantities. The synergy focuses on the antioxidant effect and/or on the improvement of the cognitive and/or executive functions in humans or animals.

The polyphenols present in the agent according to the invention, when administered to humans or animals, also have an improved bioavailability compared to polyphenols taken alone or to existing extracts containing these polyphenols in different proportions and quantities. The agent according to the invention used in humans or animals thus allows the bioavailability of the polyphenols contained in said agent to be improved.

The agent according to the invention can be used as a drug for humans or animals. In particular, the invention relates to the use of the therapeutic or nutritional agent in the treatment or prevention in humans or animals of Alzheimer's disease and/or Parkinson's disease and/or Huntington's disease and/or pathological cognitive decline and/or dementia and/or depression and/or diabetes and/or schizophrenia and/or mental retardation and/or disorders relating to the post-menopausal condition in women and/or cognitive dysfunction syndrome (CDS).

The agent according to the invention can also be used in healthy humans or animals, for a non-therapeutic use, to improve cognitive functions and/or executive functions, and/or to limit age-related non-pathological cognitive decline, preferably in a nutritional composition or a food supplement. It can in particular be used in healthy humans or animals to improve memory and/or attention and/or concentration and/or alertness and/or learning and/or intelligence and/or language and/or mood and/or stress and/or anxiety and/or outlook and or sleep.

According to a particular embodiment of the invention, the human or animal is elderly. Preferably the elderly human or animal is a human or animal who has completed at least 50% of the average lifespan for his/its species.

Preferably, the therapeutic or nutritional agent is used as a dose, a quantity that provides the sick human or animal for therapeutic uses or a healthy human or animal for non-therapeutic uses:

-   -   at least 100 μg per kg of body weight of catechin and/or         epicatechin,     -   preferably at least 0.05 μg per kg of body weight of ferulic         acid,     -   at least 10 μg per kg of body weight of resveratrol,     -   at least 0.2 μg per kg of body weight of quercetin and/or         quercetin glycosides, and     -   at least 1 μg per kg of body weight of anthocyanidins.

The invention is described here through examples and test results proving the antioxidant synergistic effect and the effect on cognitive and executive functions, and the improvement of bioavailability of the therapeutic or nutritional agent covered by the present application.

EXAMPLES Example 1: Therapeutic or Nutritional Agent According to the Invention

This first example of a mixture according to the invention is obtained by adopting the method described below.

The raw materials used are:

-   -   the skin and seeds (pips) of the fruits of Vitis vinifera,         by-products of the wine industry,     -   frozen Vaccinium angustifolium berries.

400 g of frozen Vaccinium angustifolium berries are crushed and mixed with a solution of 2000 ml of 80% (v/v) ethanol with a content of 0.1% by weight of HCl. The mixture is kept at ambient temperature (20° C.) for 24 hours. The ethanolic solution is then separated from the pulp by filtration, and under vacuum-concentrated with a rotary evaporator to 20% of dry matter. Part of this extract is preserved for testing, the other part is kept to be mixed with the extract of Vitis vinifera.

500 g of pellicle and seeds of Vitis vinifera are mixed with 2500 ml of 80% (v/v) ethanol with a 0.1% content by weight of HCl at 40° C. for 5 hours. The ethanolic solution is then separated from the pulp by filtration. The ethanol is then under vacuum removed with a rotary evaporator at a temperature of 50° C. at 60 mbars. The aqueous solution is then diluted to obtain 5% dry matter and filtered through a 5000-dalton membrane. The permeate obtained is then loaded onto a resin column (C18) at 1BV/hour. The resin is then flushed for a first time with 3BV of distilled water at 2BV/hour and then eluted with 5BV of an 80% (v/v) ethanolic solution at 1 BV/hour. Part of the extracted solution is kept for testing and is characterized (Table 1a).

The polyphenols presented in this table were measured by ultra performance liquid chromatography with a fluorescence detector.

TABLE 1a Flavanol content of the extract of Vitis vinifera Flavanol monomer and proanthocyanidin content (dry weight % - eq. Epicatechins) (measured by LC with a fluorescence detector) Monomers 35.27% ± 1.67  Dimers 22.92% ± 1.31  Trimers 8.93% ± 0.46 Tetramers 2.95% ± 0.14 Pentamers 1.09% ± 0.07 Hexamers 0.63% ± 0.14 Heptamers 0.15% ± 0.05 Octamers Not Detected Nonamers Not Detected Decamers Not Detected Polymers (Degree of Not Detected polymerization >10)

The other part is then mixed with the extract of Vaccinium angustifolium to form the mix according to the invention and a maltodextrin is added to the mix until a solution is obtained that has a dry matter content of 30%.

The solution is then spray-dried at an inlet temperature of 160° C.

The product obtained is a purple powder containing the polyphenols presented in Table 1b.

The polyphenols presented in this Table were measured by ultra-performance liquid chromatography tandem mass spectrometry (UPLC-MS/MS).

TABLE 1b Polyphenol content of the agent according to the invention of Example 1 500 mg of Equivalent in Mixture mixture/kg mg/kg (humans according to of mouse according to the the invention body weight FDA) Catechin and 25.7% 128.5 mg/kg of 10.4 mg/kg of epicatechin body weight body weight Anthocyanidins 0.436% 2.18 mg/kg of 177 μg/kg of (of which (1310 ppm) body weight body weight malvidin 3-glucoside) Quercetin and 0.864% 4.32 mg/kg of 35 μg/kg of quercetin body weight body weight glycosides Ferulic acid 0.0094% 47 μg/kg of 3.82 μg/kg of body weight body weight Resveratrol 0.0437% 218 μg/kg of 17.7 μg/kg of body weight body weight

Example 2: Therapeutic or Nutritional Agent According to the Invention

This second example of a mixture according to the invention is obtained by adopting the method described below.

The raw materials used are:

-   -   the seeds and skin of Vitis vinifera     -   Vaccinium angustifolium berries.

1000 g of frozen pomace of Vaccinium angustifolium are crushed and mixed with a solution of 5000 ml of 60% (v/v) ethanol with a content of 0.1% by weight of HCl. The mixture is kept at ambient temperature (20° C.) for 24 hours. The ethanolic solution is then separated from the pulp by filtration, and under vacuum-concentrated with a rotary evaporator to 20% of dry matter.

400 g of skin and seeds of Vitis vinifera are selected and mixed with 1500 ml of 80% (v/v) ethanol at 60° C. for 5 hours. The ethanolic solution is then separated from the pulp by filtration. The ethanol is then under vacuum-removed with a rotary evaporator at a temperature of 50° C. at 60 mbars. The aqueous solution is then diluted to give 5% dry matter and filtered through a 5000-dalton membrane. The permeate obtained is then loaded onto a resin column (C18) at 1BV/hour. The resin is then flushed for a first time with 3BV of distilled water at 2BV/hour and then eluted with 5BV of an 80% (v/v) ethanolic solution at 1 BV/hour. Part of the extracted solution is kept for testing and characterization (Table 2a).

TABLE 2a Flavanol content of the extract of Vitis vinifera Flavanol monomer and proanthocyanidin content (dry weight % - eq. Epicatechins) (measured by LC with a fluorescence detector) Monomers  9.4% ± 0.8 Dimers  4.0% ± 0.3 Trimers 0.81% ± 0.1 Tetramers 0.24% ± 0.1 Pentamers Not Detected Hexamers Not Detected Heptamers Not Detected Octamers Not Detected Nonamers Not Detected Decamers Not Detected Polymers (Degree of Not Detected polymerization >10)

The product obtained is a purple powder containing the polyphenols presented in Table 2b. The polyphenols presented in this Table were measured by ultra-performance liquid chromatography tandem mass spectrometry (UPLC-MS/MS).

TABLE 2b Polyphenol content of the agent according to the invention of Example 2 Equivalent in Mixture 4 mg of mixture/ mg/kg (humans according to the kg of mouse according to the invention body weight FDA) Catechin and 9.4% 376 μg/kg of 124 μg/kg of epicatechin body weight body weight Anthocyanidins 700 ppm 2.8 μg/kg of 1.6 μg/kg of (of which (328 ppm) body weight body weight malvidin 3-glucoside) Quercetin and 77 ppm 0.37 μg/kg of 0.21 μg/kg of quercetin body weight body weight glycosides Ferulic acid 20 ppm 0.08 μg/kg of 0.044 μg/kg of body weight body weight Resveratrol 5327 ppm  21 μg/kg of 12 μg/kg of body weight body weight

Example 3: Therapeutic or Nutritional Agent According to the Invention

19.980 kg of the agent of Example 1 is mixed with 0.020 kg of colloidal silica. The composition is obtained by mixing the constituents under conventional conditions known to a person skilled in the art. The agent is placed in a PET bag, which is then placed in a box.

Example 4: Nutritional Composition Intended for Humans

Example 4 is a 400 mg capsule formed by:

-   -   Therapeutic agent of Example 1: 300 mg     -   Vitamin C: 80 mg     -   Maltodextrin: 20 mg

The composition is obtained by mixing the constituents under conventional conditions known to a person skilled in the art, and put into a capsule also according to conventional conditions. The recommended dose is 1 to 2 capsules per day.

Example 5: Drug Intended for Humans

Example 5 is a 3000 mg tablet, formed by:

-   -   Therapeutic agent of Example 1: 1500 mg     -   Sorbitol: 1400 mg     -   Red fruit flavoring: 47 mg     -   Magnesium stearate: 30 mg     -   E133 Lake Brilliant Blue FCF dye: 20 mg     -   Acesulfame K (E950): 1.5 mg     -   Sodium saccharin (E954): 1.5 mg

The composition is obtained by mixing the constituents under conventional conditions known to a person skilled in the art.

The recommended dose is 1 to 2 tablets per day.

Example 6: Nutritional Composition for Animals

The agent according to the invention of Example 2 was added to a dry extruded kibble for dogs according to AFCO standards and comprising animal meal, fat, fibers, cereals, preserving agents and antioxidants.

The addition of the agent to the kibble was performed according to several embodiments, specifically by coating and inclusion.

Coating tests were carried out by adding the agent according to the invention to a liquid palatability enhancer D′Tech Poultry (SPF, Elven, France). A first layer of poultry fat (6% in relation to the weight of the kibble) was added as a coating on the kibble, followed by a layer of mixture between the palatability enhancer (1%, 2% or 3%, the % being relative to the weight of the kibble) and the agent according to the invention (0.02%, 0.04% or 0.1%, the % being relative to the weight of the kibble).

Inclusion tests were performed by adding the agent according to the invention (0.02%, 0.04% or 0.1%, the % being relative to the weight of the kibble) to the raw material (also called premix) before extrusion.

Example 7: Veterinary Product

Gelatin capsules were prepared according to a standard procedure, by adding an agent according to the invention of Example 2 and a maltodextrin (Control: Glucidex12 Batch #421A323532, Roquette, Lestrem Cedex, France).

Evaluation of the Efficacy and Bioavailability of the Agent According to the Invention Test 1: Effect on Bioavailability in Mice

The purpose of this test is to compare the bioavailability of the polyphenols contained in the therapeutic or nutritional agent according to the invention (mixture of Example 1) with the bioavailability of the polyphenols contained in an extract of Vitis vinifera and those contained in an extract of Vaccinium angustifolium (those described in Example 1), after an acute oral (1 day) and chronic (15 days) administration to mice.

Seventy-two 4-month-old male and female mice were divided into two groups to perform the acute study and chronic study separately. In each group, three sub-groups of 10 were created, each sub-group receiving a different treatment: extract of Vitis vinifera, extract of Vaccinium angustifolium and mixture of Example 1, and a fourth sub-group of 6 mice were treated with water (control group). The treatments were administered orally by gavage. The mixture was administered at a dose of 500 mg/kg of body weight, and the extract of Vitis vinifera and the extract of Vaccinium angustifolium were administered at a dose equivalent to their quantity in the mixture dose.

-   -   Acute study: blood samples were taken from each group, before         gavage then 30 minutes after gavage for each respective         treatment. The animals were then sacrificed and blood samples         were again taken.     -   Chronic study: blood samples were collected before         supplementation (Day 0). The animals then received their         respective treatment each day, for 15 days. The last day of the         study (Day 15), 30 minutes after gavage, the animals were         sacrificed and blood samples were collected. The excrement was         collected for each mouse before and during the supplementation         period (Day 0 and Days 1 to 15 respectively). The phenolic         metabolites were extracted from samples of plasma and dry         excrement by solid-phase micro extraction (μSPE) and         characterized by UHPLC-MS/MS (ultra high-performance liquid         chromatography). The plasma concentrations of the phenolic         metabolites after acute and chronic administration of the         different treatments were compared by using Welch's statistical         test (correction of unequal variance) when the data were         presumed to be normally distributed or, when this was not the         case, by using the Mann-Whitney test, with GraphPad Prism 6.05         software. Similarly, the effects of the treatments on the         concentrations of circulating phenolic metabolites and the         concentrations accumulated in the excrement were analyzed for         pairwise comparison using Welch's statistical test if the data         were normal and the Mann-Whitney test if they were not.

Multiple comparisons were made using a variance analysis (ANOVA) or the non-parametric Kruskal-Wallis test, a test based on data following a normal or abnormal distribution. The differences were considered to be significant at p<0.05.

The ascending hierarchical classification (AHC) of the phenolic metabolites detected in the plasma and excrement of mice was achieved using MetaboAnalyst 3.0.

The results are shown in FIGS. 1 to 3 .

FIG. 1 shows the differences in bioavailability of the phenolic compounds between an acute and chronic administration of the treatments. The results are given in the form of an average±SEM *** P<0.005 versus acute supplementation. The letters “ns” in the Figure stand for Not Significant.

FIG. 1 shows that no difference is observed in the concentrations of circulating phenolic metabolites between acute supplementation and chronic supplementation for treatments with the extract of Vitis vinifera (grape) and with the extract of Vaccinium angustifolium (blueberry).

By contrast, the repeated supplementation according to the invention, i.e. extract of Vitis vinifera and extract of Vaccinium angustifolium for 15 days, is associated with an increase in the concentration of phenolic compounds in plasma (2.1 times more, p=0.0033) compared to mice receiving only one dose.

FIG. 2 shows the ascending hierarchical classification (AHC) of the phenolic metabolites analyzed in the mice before (Day 0) and after (Day 15) chronic ingestion of the three treatments.

Each line corresponds to a detected metabolite and each column to an animal studied. The squares in shades of gray indicate the intensity of the metabolite concentration in the plasma in relation to the average of all of the samples. The boxes represent the phenolic metabolites of the extract of Vaccinium angustifolium the concentration of which in the plasma increased significantly with the treatment according to the invention. The data are displayed in the form of an average±SEM **p<0.01 and p*<0.05 vs extract of Vaccinium angustifolium, B: extract of Vaccinium angustifolium, G: extract of Vitis vinifera, N: Agent according to the invention. The heat map shows that there is no difference in the concentration of circulating phenolic metabolites originating from Vitis vinifera between a supplementation with the extract of Vitis vinifera (grape) and a supplementation with the agent according to the invention, whereas the phenolic metabolites originating from Vaccinium angustifolium were found more extensively in the mouse plasma in the case of supplementation with the agent according to the invention than in the case of supplementation with the extract of Vaccinium angustifolium (blueberry). In fact, as can be seen in the boxes, whereas the same quantity of extract of Vaccinium angustifolium was administered in both cases, with the agent according to the invention, there was an increase in the absorption of the phenolic compounds of Vaccinium angustifolium of 3.0 to 5.5 times. This increase, although smaller (2.3 to 2.8 times) was also observed after acute supplementation with the agent according to the invention versus the extract of Vaccinium angustifolium.

FIG. 3 shows the AHC heat map of the phenolic metabolites analyzed in the mouse excrement before (Day 0) and after (Days 1 to 15) chronic ingestion of extract of Vaccinium angustifolium (blueberry), extract of Vitis vinifera (grape), and the agent according to the invention.

Each line corresponds to the metabolite detected and each column to an animal studied. The squares in shades of gray indicate the intensity of the phenolic metabolite concentration in the excrement in relation to the average of the samples. The boxes represent the phenolic metabolites of Vaccinium angustifolium the concentration of which in the excrement decreased significantly when the agent according to the invention was ingested versus the extract of Vaccinium angustifolium. The results are given as an average±SEM *** p<0.005 and p*<0.01 versus extract of Vaccinium angustifolium, B: extract of Vaccinium angustifolium, G: extract of Vitis vinifera, N: Agent according to the invention. As observed in the blood samples, no difference was found for the phenolic metabolites of Vitis vinifera between supplementation with the agent according to the invention and supplementation with the extract of Vitis vinifera, whereas the phenolic metabolites of Vaccinium angustifolium were found at significantly lower concentrations in the excrement of mice supplemented with the agent according to the invention in comparison to supplementation with the extract of Vaccinium angustifolium. In fact, as can be seen in the boxes, and in line with the previous observations showing an increase in the absorption of the phenolic metabolites of Vaccinium angustifolium, in the case of supplementation with the agent according to the invention, it will be observed here too that this supplementation is associated with a reduction in the excretions of the phenolic compounds of Vaccinium angustifolium of 2.9 to 6.3 times.

All of these results show that there are synergistic interactions between the extracts of Vaccinium angustifolium and Vitis vinifera leading to an increase in bioavailability.

Test 2: Bioavailability in Mice Brains

The purpose of this study is to determine whether polyphenols and their metabolic derivatives are capable of accessing the central nervous system, in order to know whether they have effects on the brain.

In order to evaluate the presence of polyphenols in the brain, 6 control mice (3 adults and 3 aged) and 20 supplemented mice (10 adults and 10 aged) were fed with a controlled food free of polyphenols or with a food enriched with the agent according to the invention (Example 1) for 6 weeks. The dose of the agent according to the invention was 500 mg/kg of body weight/day. The mouse brains were recovered at the end of the experiment, dissected and stored at −80° C. The specific polyphenols and metabolites were measured by ultra performance liquid chromatography UPLC-MS/MS.

The results are shown in Table 3 below and in FIGS. 4A to 4D.

TABLE 3 Quantity of polyphenols detected in mice brains Agent Agent Control Control according to according to Content of Adult Aged the invention the invention brain, pmol/g Mice Mice Adult Mice Aged Mice Epicatechin 0 0 3.54 ± 4.99  8.84 ± 15.40 Catechin 0 0 0.95 ± 1.45  7.12 ± 10.45 PAC-B Dimers 0 0 2.70 ± 4.52 5.82 ± 8.33 Methyl-catechin 0 0 5.60 ± 8.56 3.15 ± 3.54 glucuronide Catechin 0 0 0.81 ± 1.85 1.47 ± 1.88 glucuronide Ferulic Acid 0 0 0.80 ± 2.01 0.42 ± 0.96

After 6 weeks of consuming a food enriched with the agent according to the invention, catechins and epicatechins and their metabolites (methyl-catechin glucuronide, catechin-glucuronide) and ferulic acid were found in the mouse brains. Dimers of proanthocyanidins were also found. These polyphenols were not found in the brains of the control mice. No significant difference was found as regards age. The polyphenols of the agent according to the invention, due to their particular association and their specific quantity can reach the brain directly to produce their neuroprotective effects.

Test 3: Properties of Polyphenols in a Neuronal Cell Culture Model

Like epicatechins, catechin and ferulic acid were detected in the brain. The aim of this study is to test their ability to protect neuronal cells and their potential synergistic effect by using different experimental models.

For this, SK-N-SH cells, a cell line of human neuroblasts, were kept in a MEM supplemented with 10% (v/v) FBS, 100 U/ml of penicillin, 100 μg/ml of streptomycin and 1% sodium pyruvate (1 mM) in a humidified incubator at 37° C. with 5% CO₂. The cells were grown to 80% confluence then seeded in multi-well cell culture plates to create different experimental models. The neuroprotective effect of the different compounds was analyzed by two different and complementary tests: the cell death quantification test and the cell survival test.

The cell death test is a colorimetric test based on measuring the activity of the lactate dehydrogenase (LDH) released by the cytosol from damaged cells in the supernatant.

The cell survival test was performed by conducting a Resazurin Test. Resazurin is an oxidation-reduction indicator of the permeable cell that can be used to monitor the number of viable cells by using tetrazolium compounds. The viable cells with an active metabolism can reduce resazurin into a resorufin product that is pink and fluorescent.

SK-N-SH neuronal cells were subjected to a toxic concentration of hydrogen peroxide (250 μM) and co-treated with epicatechin, catechin or ferulic acid at 1 μM, 1 nM and 1 pM for 24 hours. On completing the treatment, the cells were washed twice and cell death (release of LDH) and survival (Resazurin test) were analyzed. The results showing the effects of the three polyphenols taken individually after this acute treatment are shown in FIG. 5A. It will be observed that the polyphenols taken individually do not protect the cells against hydrogen peroxide.

In order to study the synergistic effect of epicatchin, catechin and ferulic acid, the SK-N-SH neuronal cells were subjected for 24 hours to a toxic concentration of hydrogen peroxide and co-treated with a mix comprising epicatechin, catechin and ferulic acid, said mix being tested at the different concentrations of 1 μM, 1 nM or 1 pM. On completing the treatment, the cells were washed twice and the cell death (release of LDH) and survival (Resazurin test) were analyzed. The results showing the effects of three polyphenols combined after this acute treatment are presented in FIG. 5B. It will be observed that the combination of the three polyphenols does not protect the cells against hydrogen peroxide.

The neuroprotective effects of the three polyphenols, i.e. epicatechin, catechin and ferulic acid, with a cumulative treatment, were then studied. The SK-N-SH cells were grown to 80% confluence then seeded in multi-well cell culture plates. On the following day, each of the three polyphenols were added separately to the 1 μM, 1 nM and 1 pM medium for 3 consecutive days. On the third day, the cells were subjected to a toxic concentration of hydrogen peroxide (250 μM) and the protection was analyzed 24 hours later. On completing the treatment, the cells were washed twice and cell survival (Resazurin test) was analyzed. The results showing the effects of the three polyphenols taken individually (the mix) after this cumulative treatment are shown in FIG. 5C. It will be observed that the polyphenols taken individually do not protect the cells against hydrogen peroxide after 3 days of consecutive treatment.

In order to study the synergistic effect of epicatechin, catechin and ferulic acid, the SK-N-SH cells were grown to 80% confluence then seeded in multi-well cell culture plates. On the following day, a mix of three polyphenols was added to the medium for 3 consecutive days, each polyphenol being present at a concentration of 1 μM, 1 nM or 1 pM in the mix. On the third day, the cells were subjected to a toxic concentration of hydrogen peroxide (125 μM and 250 μM) and the protection was analyzed 24 hours later. On completing the treatment, the cells were washed twice and cell survival (Resazurin test) was analyzed. The results showing the effects of the mix of three polyphenols after this cumulative treatment are shown in FIG. 5D. It will be observed that the mix of epicatechin, catechin and ferulic acid at 1 μM or 1 nM or 1 pM protects the cells against hydrogen peroxide after 3 days of consecutive treatment. The same test was performed with weaker concentrations in the mix of three polyphenols: 10⁻¹⁵ M, 10⁻¹⁵ M or 10⁻²¹ M of each polyphenol in the mix. It will be observed in FIG. 5E that with these weaker concentrations, the mix does not protect the cells against toxic hydrogen peroxide concentrations. This clearly shows that the quantity of three specific polyphenols in the agent according to the invention is important to achieve the desired synergistic effect.

As the mix of three polyphenols in sufficient quantity is capable of protecting the SK-N-SH neuronal cells after a cumulative treatment, a study of the effect of the mix on the intracellular production of ROS (Reactive Oxygen Species) was then carried out. For this, the cells were grown to 80% confluence then seeded in multi-well cell culture plates. On the following day, a mix containing three polyphenols, i.e. epicatechin, catechin and ferulic acid was added to the medium, each polyphenol being present at a concentration of 1 μM, 1 nM or 1 pM in the mix. On the third day, the SK-N-SH cells were subjected to a toxic concentration of hydrogen peroxide (250 μM) and the level of ROS in the cells was measured using a DCFDA fluorescent probe. The results obtained presented in FIG. 5F show that the mix of three polyphenols containing 1 μM, 1 nM or 1 pM of each of the polyphenols, enables the level of ROS to be reduced in the presence of 250 μM of hydrogen peroxide.

Test 4: Evaluation of the Synergistic Effect in Dogs of the Agent According to the Invention

The purpose of this test is to check the efficacy of an agent according to the invention (mix of Example 2) on the antioxidant status of adult dogs by comparing this efficacy to that of an extract of Vitis vinifera, an extract of Vaccinium angustifolium and a control.

Nine beagles (6 males and 3 females, BCS (body condition score) 5/9, average age 20±0.9 months, average weight 9.1±0.4 kg) were fed on a maintenance regime to maintain their body weight. The dogs' food was supplemented with gelatin capsules (Cooper, Melun Cedex, France) containing either:

-   -   a maltodextrin (Control placebo: Glucidex12 Batch #421A323532,         Roquette, Lestrem Cedex, France),     -   an extract of Vitis vinifera (Grape: Neurogrape Inside PC PR120         BatchA150288, Activ′Inside, Libourne, France),     -   an extract of Vaccinium angustifolium (Wild blueberry extract         0.4TP Batch #294, Nutra Canada, Quebec, Canada),     -   the mix of Example 2 (4 mg/kg of body weight/day).

The experiment was designed as a crossover study where the dogs were fed with experimental rations with the supplementation capsule for 28 days with a one week of wash out between each supplementation period. Each dog thus received each of the four supplementations. Blood samples were taken from the jugular vein before and after each supplementation and were kept in ice. The plasma was recovered by centrifugation at 2124 g of total blood for 10 min at 4° C. Aliquots of plasma were incubated at 80° C.

The oxidant status was evaluated by measuring the total antioxidant status (TAS). For this, a colorimetric-based assay available from RANDOX Laboratories (Ref. NX2332, Crumlin, County Antrim, UK) was used to evaluate the TAS. The method involves incubating 2,2′-Azino-di-[3-ethylbenzthiazoline sulfonate] (ABTS) with a peroxidase (metmyoglobin) and hydrogen peroxide to produce the ABTS⁺ radical cation. It has a relatively stable blue/green color, measured at 600 nm. The presence of antioxidants in the samples causes suppression of this color production to a degree which is proportional to their concentration. The TAS is expressed in mmol/L.

In order to compare the four regimes with one another, the ΔTAS was determined by comparing the TAS before and after supplementation: ΔTAS=Day 28 TAS-Baseline TAS. The ΔTAS was analyzed by using a mixed-effect model. This model includes the fixed categorical effects of the Baseline, the treatment and the randomization order. It was implemented with SAS (v9.4) software, a mixed procedure with an unstructured correlation matrix to model the within-animal errors. Parameters were estimated using the restricted maximum likelihood method with the Newton-Raphson algorithm. Denominator degrees of freedom were estimated using the Satterthwaite approximation. All the effects were evaluated with an a degree=0.10.

The Wilcoxon test was used to compare changes in the TAS value before and after supplementation.

The results obtained are presented in Table 4 (mean, standard error and Wilcoxon test) and in FIG. 6 .

TABLE 4 TAS (mmol/L) (Mean ± SEM) for groups of adult dogs (n = 9) fed on different supplementation regimes: agent according to the invention (Invention) extract of Vitis vinifera (Vv), extract of Vaccinium angustifolium (Vo) or maltodextrin (Control) for 28 days. Day 0 Day 28 p-value Standard Standard (Wilcoxon) Mean Error Mean Error Treatment TAS Va 0.92 0.122 0.90 0.109 NS mmol/L Invention 0.81 0.052 0.93 0.070 0.023 Vv 0.97 0.155 0.87 0.077 NS Control 0.84 0.048 0.88 0.075 NS

It will be observed in the Table and FIG. 6 that the mix according to the invention increases significantly and synergistically the TAS concentration compared to the extract of Vitis vinifera or the extract of Vaccinium angustifolium on their own.

Moreover, the results of the Wilcoxon test show that the invention is the only supplementation that presents significantly higher TAS concentrations after supplementation. Supplementation with extracts of Vitis vinifera or extract of Vaccinium angustifolium on their own do not significantly change the TAS concentration.

Thus, supplementation with a mix of molecules from Vitis vinifera and from Vaccinium angustifolium according to the invention has a synergistic effect on the total antioxidant status of animals compared to supplementations with an extract of Vitis vinifera and an extract of Vaccinium angustifolium taken alone.

Test 5: Evaluation of the Effect on the Memory

The purpose of this study is to check the effect of a double dose of mix according to the invention (Example 2) on the memory levels of dogs.

The study is a blind randomized preclinical study in which a longitudinal parallel group model was used. Thirty-five beagles (Vivocore Inc. Company, Toronto, Canada; 14 males and 21 females; aged between 8.0 and 14.5 years at the beginning of the study) were allocated in three groups for the experiment, three weeks before the start of the supplementations. The allocation of the dogs was determined by performance levels (cumulative scores) based on DNMP (Delayed Non-Matching Position) test scores, so that each group had a substantially equivalent total DNMP test score.

The three groups of dogs were then fed respectively with kibbles containing in inclusion either 0 ppm (placebo), or 240 ppm of the mix of Example 2, or 480 ppm of the mix of Example 2 (ppm relative to the kibble weight).

The DNMP test was performed from Day −27 to −16 and the analysis was performed from Day 58 to 63.

The DNMP test comprises two phases:

-   -   Phase 1: the dog must move an object placed in one of three         possible positions on a food well. The block to be removed         covers a reward.     -   Phase 2: after a 20 s to 90 s attempt, two objects identical to         the first phase are presented to the dog. One object is located         in the same position as in the first phase. However, the correct         object is placed in one of the two remaining positions (non         match), and if the dog moves this object, he receives the         reward.

For the present study, 12 DNPM test sessions were carried out, with one test session per day for all of the subjects. The variable-delay subtask was used. For each test session, delays of 20 and 90 seconds were equally distributed over the 12 tests, enabling evaluation of working memory. An inter-test interval of 30 seconds was applied. There were 6 sessions for the initial phase and six sessions for the treatment phase. The subjects were tested on each of the designated days, regardless of the score.

Throughout all the test procedures, the animals were rewarded with Purina Essential Care Adult Formula tinned wet dog food.

In order to compare the three treatments to the DNMP results, the increase in relation to the Baseline was analyzed using a Chi-squared test. The analysis was performed using SAS (v9.4) software with a significant level of α=0.05.

The results are presented in FIG. 7 . A significant cognitive increase was observed when the dogs received a treatment according to the invention (Mix 2) compared to dogs that did not receive the treatment. Moreover, the quantity of treatment did not affect the number of dogs showing a significant increase, which proves that, in dogs, the effectiveness is independent of the treatment dose.

Test 6: Evaluation of the Effect on a Dog's Tolerance

The purpose of this test is to check the food safety of the nutritional or therapeutic food agent of the invention on dogs, by checking certain renal biomarkers. Indeed, numerous publications have reported a toxicity of grapes in dogs, causing them renal deficiencies the symptoms of which are manifested as vomiting, diarrhea, etc. (Eubig P, Brady M, Gwaltney-Brant S, Khan S, Mazzaferro E, Morrow C (2005). “Acute renal failure in dogs after the ingestion of grapes or raisins: a retrospective evaluation of 43 dogs” (1992-2002).

Twenty-four beagles (20 males and 4 females, BCS 5/9, average age 31±3 months, average weight 11.4±0.2 kg), were fed on a maintenance food regime (Royal Canin Medium Adult, France) in order to maintain their optimal weight during the test. Four groups of 6 dogs thus each received supplements, i.e. capsules containing maltodextrin (placebo) or an agent according to the invention, i.e. the mix as prepared in Example 2: 4 (Mix 1), 20 (Mix 5), and 40 (Mix 10) mg/kg of body weight/day.

Urine and blood samples were taken at the start of the test (Week 0), after 12 weeks and after 24 weeks.

The Cystatin C (CysC), clusterin and neutrophil gelatinase-associated lipocalin (NGAL) of the plasma and urine were analyzed in the blood samples (Tvarijonaviciute A, Ceron J J, Holden S L, Biourge V, Morris R I, German A J. Effect of Weight Loss in Obese Dogs on Indicators of Renal Function or Disease. J. Vet. Intern. Med. 2013; 27:31-38; Garcia-Martinez J D, Tvarijonaviciute A, Ceron J J, Calden M, Martinez-Subierla S. Urinary Clusterin as a Renal Marker in Dogs. J. Vet. Diagn. Invest. 2012; 24:301-306). Each parameter was analyzed by means of a mixed-effect model, by evaluating the effects of the baseline, day, treatment and the day x of treatment (SAS v9.4; α=0.05).

As shown in Table 5, the biomarkers were found in quantities below the upper limit obtained with the control and experimental treatments at Week 0 (plasma CysC, urinary CysC/Crea ratio, urinary clusterin/Creat ratio, NGAL plasma and urinary/Creat NGAL at 2.23 μg/mL, 156 ng/g, 443 ng/g, 47 ng/mL, 28.5 ng/g respectively).

TABLE 5 Urinary Urinary Urinary Clusterin/ NGAL/ CysC, CysC/Creat Creat NGAL, Creat μg/mL ratio, μg/g ratio, ng/g ng/mL ratio, ng/g Mean SEM Mean SEM Mean SEM Mean SEM Mean SEM Week Control 1.25 0.085 18.90 17.243 79.3 20.05 17.8 4.52 11.12 4.688 0 Mix 1 1.25 0.152 30.38 25.390 44.5 13.22 17.0 5.02 7.97 4.487 Mix 5 1.17 0.084 27.37 14.261 63.4 27.53 14.9 3.49 4.18 1.786 Mix 10 1.47 0.161 12.20 4.441 83.7 22.67 18.0 3.00 5.45 1.019 Week Control 1.18 0.075 8.25 3.156 61.1 34.07 23.8 5.21 8.42 3.690 12 Mix 1 1.27 0.173 9.83 4.594 67.9 33.33 15.3 4.69 5.68 1.934 Mix 5 1.22 0.079 5.12 1.696 39.5 17.16 12.9 2.80 4.00 1.551 Mix 10 1.35 0.099 12.93 6.086 98.7 52.59 19.7 4.03 4.72 1.552 Week Control 1.10 0.132 14.27 9.840 135.1 66.10 23.7 2.67 7.33 2.483 24 Mix 1 1.23 0.182 4.13 1.406 94.2 69.26 19.3 4.80 4.92 1.352 Mix 5 1.18 0.079 21.42 11.941 56.2 24.72 14.3 4.04 3.52 0.297 Mix 10 1.30 0.116 3.80 1.240 47.5 20.23 20.7 3.53 4.55 1.393 p- treatment NS NS NS NS NS values day NS NS NS NS NS Treatment × NS NS NS NS NS day

Adult dogs consuming the agent according to the invention therefore show no clinical signs of intolerance, even at the maximum dose tested (10 times the normal dose).

Test 7: Effect on Alzheimer's Disease

This test was performed on a heterozygote 3×Tg-AD mouse model as described for example in Arsenault D, Dal-Pan A, Tremblay C, Benett D A, Guitton M J, et al. (2013) PAK Inactivation Impairs Social Recognition in 3×Tg-AD Mice without increasing Brain Deposition of Tau and A6. The Journal of Neuroscience 33: 10729-10740.

120 non-transgenic (Non Tg) and triple transgenic (3×Tg-AD) mice aged 12 months were used for this test. Seven mice died before the test and were excluded.

In addition, an additional group of 4-month-old C57BL/6 mice was used as a control group. The agent according to the invention of Example 1 was introduced into mouse food pellets. The mice were fed for 4 months with a control food or with 500 mg of extract/kg of body weight/day (reference “Polyph1”) or 2500 mg of extracts/k of body weight/day (reference “Polyph2”).

Three months after the start of the test, behavioral analyses were conducted. After an additional month, the mice were placed under deep anesthesia and extracts of intracardiac blood were taken. They were then perfused with an intracardiac perfusion with a saline phosphate buffer containing protease inhibitors and phosphatase inhibitors. Extracts of parietal-temporal cortex were then dissected, frozen and kept at −80° C. They were then treated for ELISA, Western Blot and immunofluorescence analysis to measure the following markers: beta-amyloid (Aβ), Tau protein and BDNF (Brain-Derived Neurotrophic Factor). First of all, a cognitive decline was observed in 3×Tg-AD and non-Tg 15-month-old mice compared to non-Tg 4-month-old mice (control). In fact, for the aged mice a reduction was observed in the recognition ratio or recognition index during the novel object recognition test. Advantageously, the administration of the agent according to the invention at doses of 500 or 2500 mg/kg/day prevents the deterioration of the memory in 3×Tg-AD mice.

Furthermore, the agent according to the invention prevents the reduction of BDNF (Brain-Derived Neurotrophic Factor) in 16-month-old 3×Tg-AD mice.

Lastly, the results obtained show that phenolic metabolite concentrations are correlated with the cognitive performance (memory) of mice supplemented with the agent according to the invention. 

1. A nutritional or therapeutic agent comprising at least one molecule mix obtained from Vitis vinifera and Vaccinium angustifolium, comprising: at least 1% of catechins and/or epicatechins, the percentage being given by weight in relation to the total weight of the mix, and at least 5 ppm (parts per million in the mix) of ferulic acid.
 2. The nutritional or therapeutic agent of claim 1, wherein the molecule mix comprises at least 5% of catechins and/or epicatechins, the percentage being given by weight in relation to the total weight of the mix.
 3. The nutritional or therapeutic agent according to claim 1, wherein the molecule mix comprises at least 10 ppm (parts per million in the mix) of ferulic acid.
 4. The nutritional or therapeutic agent of claim 1, wherein the molecule mix comprises malvidin 3-glucoside at a concentration of at least 300 ppm.
 5. The nutritional or therapeutic agent of claim 1, wherein the mix is formed by: an extract of Vitis vinifera and/or an extract of Vaccinium angustifolium, and an extract obtained from Vitis vinifera and Vaccinium angustifolium.
 6. The nutritional or therapeutic agent of claim 5, wherein the extract of Vitis vinifera has a flavanol polymer content of less than 0.5% by weight of the total weight of the polyphenols of the extract.
 7. The nutritional or therapeutic agent of claim 1, wherein the molecule mix also comprises: at least 200 ppm of resveratrol, and/or at least 50 ppm of quercetin and/or quercetin glycosides, and/or at least 500 ppm of anthocyanidins.
 8. A therapeutic composition for humans or animals, the therapeutic composition comprising the nutritional or therapeutic agent of claim
 1. 9. A method for treating a human or an animal in need of treatment for Alzheimer's disease and/or Parkinson's disease and/or Huntington's disease and/or pathological cognitive decline and/or dementia and/or depression and/or diabetes and/or schizophrenia and/or mental retardation and/or disorders relating to the post-menopausal condition in women and/or cognitive dysfunction syndrome (CDS), the method comprising administering to the human or the animal the nutritional or therapeutic agent of claim
 1. 10. The method of claim 9, wherein the nutritional or therapeutic agent is administered to the human or the animal at a dose providing: at least 100 μg per kg of body weight of catechins and/or epicatechins, and at least 0.05 μg per kg of body weight of ferulic acid.
 11. The method of claim 10, wherein the dose further provides: at least 10 μg per kg of body weight of resveratrol, at least 0.2 μg per kg of body weight of quercetin and/or quercetin glycosides, and at least 1 μg per kg of body weight of anthocyanidins.
 12. A method for improving cognitive functions and/or executive functions, and/or for limiting age-related non-pathological cognitive decline in a healthy human or animal, the method comprising administering the healthy human or animal the nutritional or therapeutic agent of claim
 1. 13. The method of claim 12, wherein the nutritional or therapeutic is administered for improving memory and/or attention and/or concentration and/or alertness and/or learning and/or intelligence and/or language and/or mood and/or stress and/or anxiety and/or outlook and or sleep.
 14. The method of claim 12, wherein the nutritional or therapeutic agent is administered in a quantity providing to the healthy human or animal: at least 100 μg per kg of body weight of catechins and/or epicatechins, and at least 0.05 μg per kg of body weight of ferulic acid.
 15. The method of claim 14, wherein the nutritional or therapeutic agent is administered in a quantity providing to the healthy human or animal: at least 10 μg per kg of body weight of resveratrol, at least 0.2 μg per kg of body weight of quercetin and/or quercetin glycosides, and at least 1 μg per kg of body weight of anthocyanidins.
 16. A composition comprising the nutritional or therapeutic agent of claim 1, wherein the composition is in a form selected from tablets, capsules, gel capsules, powders, solutions, microcapsules, suspensions, emulsions, food supplements, drinks and food for humans or animals. 